%0 Journal Article
%T Studies on the Expression, Purification and Renaturation of Recombinant N_acety_L_ornithine Deacetylase<br>重组N-乙酰鸟氨酸脱乙酰基酶的表达、纯化和复性研究
%A LI Huan
%A CHEN Yue
%A WENG Qiu-Ping
%A WU Ming-Gang
%A WEI Ping
%A OUYANG Ping-Kai
%A <br>李环
%A 陈悦
%A 翁秋萍
%A 吴明刚
%A 韦萍
%A 欧阳平凯
%J 生物工程学报
%D 2007
%I 
%X The argE gene from Escherichia coli coding for N-acety-L-ornithine deacetylase(NAOase), the key enzyme involved in the L-arginine biosynthesis, had been cloned in pET22b and transformed into BL21 (DE3). With 32.5% expression level in the optimal fermentation medium at 37 degrees C, most NAOase was expressed as inclusion bodies. The soluble and active proportion could be slightly increased when expressed at low temperature. The specific activity of soluble NAOase purified by Ni-NTA resin chromatography was 1193.2u/mg. The species and proportions of whole cell proteins varied with induction conditions. The inclusion bodies expressed at 37 degrees C was more pure than 22 degrees C after gradient wash with urea. Inclusion bodies could be partly refolding and reactivated by dilution and dialysis. Low protein concentration and suitable rate of oxidant/reducing agents were important to renaturation. In the optimal conditions 17.78% of Urea-denatured NAOase could be refolding and reactivated by dilution. The purified fusion protein was obtained after wash, solubilization and Ni-NTA resin affinity chromatography purification of inclusion bodies.
%K recombinant N-acetylornithine deacetylase
%K cellular location
%K affinity purification
%K inclusion bodies
%K renaturation<br>重组N-乙酰鸟氨酸脱乙酰基酶
%K 表达定位
%K 亲和纯化
%K 包涵体
%K 复性
%U http://www.alljournals.cn/get_abstract_url.aspx?pcid=90BA3D13E7F3BC869AC96FB3DA594E3FE34FBF7B8BC0E591&jid=A66E90C274451689E69F6F0291467824&aid=310CCAE1F7D3CF37&yid=A732AF04DDA03BB3&vid=EA389574707BDED3&iid=38B194292C032A66&sid=036D726259190A01&eid=4A2356A1257A12EB&journal_id=1000-3061&journal_name=生物工程学报&referenced_num=4&reference_num=11